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Bio-protocol 11(05): e3942. 
DOI:10.21769/BioProtoc.3942

 
 

 
Generation and Implementation of Reporter BHK-21 Cells for Live Imaging of Flavivirus 

Infection 

Jorge L. Arias-Arias and Rodrigo Mora-Rodríguez*  

 

Centro de Investigación en Enfermedades Tropicales, Facultad de Microbiología, Universidad de Costa 
Rica, San José, 11501-2060, Costa Rica 

*For correspondence: rodrigo.morarodriguez@ucr.ac.cr 

 
[Abstract] The genus Flavivirus within the family Flaviviridae includes many viral species of medical 

importance, such as yellow fever virus (YFV), Zika virus (ZIKV), and dengue virus (DENV), among 

others. Presently, the identification of flavivirus-infected cells is based on either the immunolabeling of 
viral proteins, the application of recombinant reporter replicons and viral genomes, or the use of cell-

based molecular reporters of the flaviviral protease NS2B-NS3 activity. Among the latter, our flavivirus-
activatable GFP and mNeptune reporters contain a quenching peptide (QP) joined to the fluorescent 

protein by a linker consisting of a cleavage site for the flavivirus NS2B-NS3 proteases (AAQRRGRIG). 
When the viral protease cleaves the linker, the quenching peptide is removed, and the fluorescent 

protein adopts a conformation promoting fluorescence. Here we provide a detailed protocol for the 
generation, selection and implementation of stable BHK-21 cells expressing our flavivirus genetically-

encoded molecular reporters, suitable to monitor the viral infection by live-cell imaging. We also describe 
the image analysis procedures and provide the required software pipelines. Our reporter cells allow the 

implementation of single-cell infection kinetics as well as plaque assays for both reference and native 
strains of flaviviruses by live-cell imaging. 

 
Graphic abstract: 

 
Workflow for the generation and implementation of reporter BHK-21 cells for live imaging of 
flavivirus infection. 

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mailto:rodrigo.morarodriguez@ucr.ac.cr


                 

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Keywords: Flavivirus, Fluorescence, NS2B-NS3, Protease, Live-cell imaging, Reporter cells, Plaque 

assay, Image analysis 
 

[Background] Flaviviruses represent an emerging and re-emerging global threat that cause diseases 

both in animals and humans, including many medically relevant viruses like yellow fever virus (YFV), 

West Nile virus (WNV), Japanese encephalitis virus (JEV), dengue virus (DENV), and Zika virus (ZIKV), 

among others (Gould and Solomon, 2008). At present, the detection of flavivirus-infected cells is based 

on either the antibody labeling of viral proteins (Balsitis et al., 2008), the use of recombinant reporter 

replicons and viral genomes (Li et al., 2013; Schmid et al., 2015; Xie et al., 2016; Tamura et al., 2017; 

Kümmerer, 2018), or the application of genetically-encoded molecular reporters of the flavivirus NS2B-

NS3 proteolytic activity (Medin et al., 2015; Hsieh et al., 2017; McFadden et al., 2018). Immunolabeling 

implies both fixation and permeabilization which hamper their implementation for studies in living cells. 

Reporter replicons and viral genomes are suitable for live-cell imaging assays, but they are restricted to 

particular molecular clones mainly derived from reference strains and thus, not applicable when working 

with clinical isolates or native viral strains. In this context, cell-based molecular reporters of the flaviviral 

proteases constitute a favorable alternative for the study of native flavivirus strains by live-cell imaging. 

Based on our recently published flavivirus-activatable GFP (FlaviA-GFP) and flavivirus-activatable 

mNeptune (FlaviA-mNeptune) reporters (Arias-Arias et al., 2020), here we describe in detail a protocol 

for the generation, selection, and implementation of stably-transduced reporter BHK-21 cells for live 

imaging of flavivirus infection in single cells and viral plaques. Furthermore, we provide a rationale for a 

software-based image analysis approach to demonstrate the capabilities of this reporter cell line for 

single-cell and viral-plaque tracking. In addition, we include the optimized CellProfiler analysis pipelines 

for studies employing this or other cell-based reporters. Our approach represents the first fluorescence 

activatable cell-based reporter system for monitoring the kinetics of infection by both reference and 

native strains of flaviviruses like DENV, ZIKV, and YFV using live-cell imaging.   
 
Materials and Reagents 
 

1. Cell culture flasks, 75 cm2 (Greiner Bio-One, CELLSTAR®, catalog number: 658175) 
2. Cell culture dishes, 100/20 mm (Greiner Bio-One, CELLSTAR®, catalog number: 664160) 

3. 2 ml reaction tubes (Greiner Bio-One, catalog number: 623201) 
4. 3 ml sterile syringes (Ultident Scientific, catalog number: BD-309657) 

5. Syringe filters 0.2 μm hydrophilic polyethersulfone, 32 mm diameter (Pall, Acrodisc®, catalog 
number: 4652) 

6. 10 ml sterile syringes (Ultident Scientific, catalog number: BD-302995) 
7. Syringe filters 0.45 μm hydrophilic cellulose acetate, 28 mm diameter (Sartorius, Minisart®, 

catalog number: 16555) 

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8. 15 ml conical tubes (Greiner Bio-One, CELLSTAR®, catalog number: 188271) 

9. 0.5 ml reaction tubes (Greiner Bio-One, catalog number: 667201) 
10. Hexadimethrine bromide (Merck, Sigma-Aldrich, catalog number: H9268) 

11. 48-well cell culture plates (Greiner Bio-One, CELLSTAR®, catalog number: 677180) 
12. 1.5 ml reaction tubes (Greiner Bio-One, catalog number: 616201) 

13. 12-well cell culture plates (Greiner Bio-One, CELLSTAR®, catalog number: 665180) 
14. 1.5 ml light protection reaction tubes (Greiner Bio-One, catalog number: 616283) 

15. Cell culture flasks, 25 cm2 (Greiner Bio-One, CELLSTAR®, catalog number: 690175) 
16. 6-well cell culture plates (Greiner Bio-One, CELLSTAR®, catalog number: 657160) 

17. 96-well black cell culture plates (Greiner Bio-One, µCLEAR®, catalog number: 655096) 
18. 24-well cell culture plates (Greiner Bio-One, CELLSTAR®, catalog number: 662160)  

19. HEK 293T cells (ATCC, catalog number: CRL-3216)  
20. Plasmids:  

pLenti-FlaviA-GFP-puro (a gift from Jorge L. Arias-Arias, Addgene plasmid #140088) 
pLenti-CMV-FlaviA-mNeptune-puro (a gift from Jorge L. Arias-Arias, Addgene plasmid #140091)  

pMD2.G (a gift from Didier Trono, Addgene plasmid #12259) 
psPAX2 (a gift from Didier Trono, Addgene plasmid #12260) 

21. LB agar plates with 100 µg/ml ampicillin (Merck, Sigma-Aldrich, catalog number: L5667) 
22. LB broth (Miller) (Merck, Sigma-Aldrich, catalog number: L2542) 

23. 100 mg/ml ampicillin solution (Merck, Sigma-Aldrich, catalog number: A5354) 
24. NucleoSpin plasmid mini kit (Macherey-Nagel, catalog number: 740588.50) 

25. DMEM, high glucose, GlutaMAXTM, pyruvate (Thermo Fisher Scientific, Gibco, catalog number: 
10569044) 

26. Antibiotic-antimycotic 100× (Thermo Fisher Scientific, Gibco, catalog number: 15240062) 
27. Fetal bovine serum (FBS) qualified, heat inactivated (Thermo Fisher Scientific, Gibco, catalog 

number: 10438-026) 
28. Polyethylenimine (PEI), linear, MW 25000, transfection grade (Polysciences, PEI 25KTM, catalog 

number: 23966-1) 
29. UltraPureTM DNase/RNase-free distilled water (Thermo Fisher Scientific, Invitrogen, catalog 

number: 10977015) 
30. Hydrochloric acid, 36.5-38.0%, BioReagent (Merck, Sigma-Aldrich, catalog number: H1758) 

31. BHK-21 [C-13] (ATCC, catalog number: CCL-10)  
32. MEM, GlutaMAXTM supplement (Thermo Fisher Scientific, Gibco, catalog number: 41090101). 

33. Sodium pyruvate, 100 mM (Thermo Fisher Scientific, Gibco, catalog number: 11360070). 
34. PBS, pH 7.4 (Thermo Fisher Scientific, Gibco, catalog number: 10010023). 

35. TrypLETM express enzyme (1×), no phenol red (Thermo Fisher Scientific, Gibco, catalog number: 
12604013) 

36. Puromycin dihydrochloride from Streptomyces alboniger (Merck, Sigma-Aldrich, catalog 

number: P8833) 

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37. Clinical isolate DENV-2/CR/13538/2007 (Instituto Costarricense de Investigación y Enseñanza 
en Nutrición y Salud, Cartago, Costa Rica) (Soto-Garita et al., 2016) 

38. Vaccine strain YFV/US/17D/1937 (Sanofi Pasteur, YF-VAX®)   

39. FluoroBriteTM DMEM (Thermo Fisher Scientific, Gibco, catalog number: A1896701) 
40. GlutaMAXTM supplement (Thermo Fisher Scientific, Gibco, catalog number: 35050061) 

41. Minimum essential medium eagle AutoModTM (Merck, Sigma-Aldrich, catalog number: M0769) 
42. Carboxymethylcellulose sodium salt (Merck, Sigma-Aldrich, catalog number: C4888) 

43. Sodium bicarbonate (Merck, Sigma-Aldrich, catalog number: S5761) 
44. Complete DMEM (see Recipes) 

45. PEI solution (1 mg/ml) (see Recipes) 
46. Polybrene solution (10 mg/ml) (see Recipes) 

47. Complete MEM (see Recipes) 
48. PBS 1% FBS (see Recipes) 

49. Puromycin solution (10 mg/ml) (see Recipes) 
50. FluoroBriteTM DMEM 2% FBS (see Recipes) 

51. Plaque media 2% FBS (see Recipes) 

 
Equipment 
 

1. Biological safety cabinet (ESCO, Labculture® Class II, Type A2, catalog number: LA2-3A2-E) 

2. CO2 incubator (Thermo Scientific, model: Forma Series II, catalog number: 3110) 
3. 4 °C refrigerator (Thermo Scientific, Value Lab, catalog number: 20LREETSA) 

4. -20 °C freezer (Thermo Scientific, Value Lab, catalog number: 20LFEETSA) 
5. -80 °C freezer (Sanyo, VIP series, catalog number: MDF-U32V) 

6. Water bath (PolyScience, catalog number: WBE20A12E) 
7. Centrifuge (Eppendorf, model: 5810) 

8. Microcentrifuge (Eppendorf, model: 5418) 
9. Pipettes (Thermo Scientific, FinnpipetteTM F2 GLP Kit, catalog number: 4700880) 

10. Pipet filler (Thermo Scientific, S1, catalog number: 9511) 
11. Hemocytometer (Boeco, Neubauer improved, catalog number: BOE 13)   

12. Shaking incubator (Shel Lab, catalog number: SSI3)  
13. ThermoMixer® C block (Eppendorf, catalog number: 5382000015) 

14. Vortex mixer (Thermo Scientific, MaxiMixTM, catalog number: M16715Q) 
15. Ultraviolet crosslinker (UVP, CL-100, catalog number: UVP95017401) 

16. NanoDropTM 2000 spectrophotometer (Thermo Scientific, catalog number: ND-2000) 
17. Steam sterilizer (Yamato, catalog number: SQ510) 

18. Water purification system (Merck, Milli-Q advantage A10) 
19. Inverted microscope (Nikon, Eclipse, catalog number: TS100) 

20. Flow cytometer (BD Biosciences, BD AccuriTM C6)  

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21. Cell sorter (BD Biosciences, BD FACSJazzTM)  

22. Automated fluorescence microscope (Biotek, Lionheart FX) with: 
CO2 gas controller (Biotek, catalog number: 1210012) 

Humidity chamber (Biotek, catalog number: 1450006) 
4× objective (Biotek, catalog number: 1220519) 

20× objective (Biotek, catalog number: 1220517) 
GFP filter cube (Biotek, catalog number: 1225101) 

465 nm LED cube (Biotek, catalog number: 1225001) 
Cy5 filter cube (Biotek, catalog number: 1225105) 

623 nm LED cube (Biotek, catalog number: 1225005) 
 
Software 
 

1. Gen5 Image+ (Biotek, https://www.biotek.com) 
2. CellProfiler 4.0 (Broad Institute, https://cellprofiler.org/releases) 

 
Procedure 
 

A. Lentiviral vectors assembly and titration 
Assembly 

1. Prepare plasmid stocks following standard molecular biology procedures 
(https://www.jove.com/v/5062/plasmid-purification) and the protocol provided by the 

manufacturer of the NucleoSpin plasmid mini kit (Macherey-Nagel).  
2. Manually seed 6,000,000 HEK 293T cells in 100/20 mm cell culture dishes with 8 ml of DMEM 

10% FBS (Recipe 1) and incubate overnight at 37 °C and 5% CO2 to reach 70-80% confluency. 
For a detailed procedure of seeding cells please refer to the bio-protocol paper by Freppel et 

al., 2018 (reference 3). 

3. Using a pipette, replace the medium by removing and discarding all the DMEM 10% FBS in the 

dishes (~8 ml) and adding 4 ml of fresh DMEM 2% FBS (Recipe 1). 
4. Prepare the transfection mix as follows:  

Suspension A: 45 µl PEI 1 mg/ml (Recipe 2) + 955 µl unsupplemented DMEM (without FBS and 
antibiotic-antimycotic).   

Suspension B: 6 µg pLenti-FlaviA-GFP-puro or pLenti-CMV-FlaviA-mNeptune-puro + 6 µg 
pMD2.G + 6 µg psPAX2 and bring to 1,000 µl with unsupplemented DMEM.  

Mix suspensions A with B and incubate for 15 min at room temperature.  
5. Add the 2 ml transfection mix to the cells (dropwise) and incubate overnight at 37 °C and 5% 

CO2. 
6. Replace the medium with 6 ml of fresh DMEM 2% FBS and incubate for 48 h at 37 °C and 5% 

CO2. 

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7. Harvest culture supernatants and filter them (0.45-μm pore size) to eliminate cells and debris. 

Use filters with low protein adherence, like cellulose acetate or polyethersulfone (PES). Do not 
use nitrocellulose filters as they could bind the lentiviral particles.   

8. Prepare 500 µl aliquots and store at -80 °C.  
 

Titration  

1. As described above, seed 50,000 BHK-21 cells per well in a 48-well cell culture plate with 500 

µl/well of MEM 2% FBS (Recipe 4) and incubate overnight at 37 °C and 5% CO2. Prepare extra 
wells to be used as control cells. 

2. Thaw in a water bath (37 °C) one of the lentiviral 500 µl stock aliquots and add polybrene 
(Recipe 3) at a final concentration of 5 µg/ml. 

3. Prepare 10-fold serial dilutions (10-1-10-6) of the lentiviral stock in 1.5 ml reaction tubes. Start 
mixing 50 µl of the lentiviral particles in 450 µl of DMEM 2% FBS + 5 µg/ml polybrene (10-1). 

Vortex the tube for 5 s and mix 50 µl of the 10-1 lentiviral dilution in 450 µl of DMEM 2% FBS + 
5 µg/ml polybrene (10-2). Repeat this procedure for the other dilutions (10-3-10-6) and incubate 

for 15 min at room temperature. Change the tip between dilutions to avoid cross-contamination. 
For a detailed and graphical explanation of 10-fold serial dilutions preparation please refer to 
the bio-protocol paper by Freppel et al., 2018 (reference 3). 

4. Replace the medium of the cells with 150 µl/well of undiluted lentiviral stock and each serial 

dilution thereof. Add 150 µl/well of DMEM 2% FBS + 5 µg/ml polybrene to the control cells. To 
avoid cross contamination, make the inoculation of the samples in order, starting with the control, 

following with the serial dilutions (from higher to lower dilution), and ending with the undiluted 
lentiviral stock.  

5. Centrifuge at 300 × g for 2 h at 25 °C for viral adsorption.  

6. Replace the inoculum with 500 µl/well of DMEM 2% FBS and incubate for 48 h at 37 °C and 5% 

CO2. 
7. Discard the medium, wash the cells once with 100 µl/well of PBS, add 100 µl/well of TrypLETM 

express (no phenol red), incubate for 5 min at 37 °C, and resuspend the cells with 400 µl/well 
of PBS 1% FBS (Recipe 5).  

8. Based on the basal background of the reporter proteins and by comparison with the non-
transduced control cells (Figure 1), determine by flow cytometry the percentage of GFP+ (488 

nm laser - 530/30 nm filter) or mNeptune+ (640 nm laser -675/25 nm filter) cells present in the 
samples infected with different dilutions of the lentiviral seed. For a detailed procedure about 
flow cytometry of fluorescent proteins please refer to the protocol by Hawley et al., 2004 

(reference 5).   

9. Using the data of the higher dilution with detectable transduced cells, calculate the biological 
titer in transducing units per milliliter (TU/ml), applying the following formula:  

TU/ml = (P × N / 100 × V) × 1/DF 
 

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where P = % GFP+ or mNeptune+ cells, N = number of cells at transduction = 50,000, V = 

volume of inoculum per well = 0.15 ml, and DF = dilution factor = 1 (undiluted), 10–1 (diluted 
1/10), 10–2 (diluted 1/100), and so on (Tiscornia et al., 2006). 

 
B. Reporter cell lines production and selection 

Production 

1. As described above, seed 100,000 BHK-21 cells per well in a 12-well cell culture plate with 1 

ml/well of MEM 2% FBS and incubate overnight at 37 °C and 5% CO2. Prepare an extra well 
for the control cells. 

2. Thaw in a water bath (37 °C) one of the 500 µl stock aliquots of lentiviral particles carrying 
genetic constructs codifying for either the FlaviA-GFP or the FlaviA-mNeptune reporters and 

add polybrene at a final concentration of 5 µg/ml. 
3. Based on the previously calculated biological titer in TU/ml, prepare 500 µl/well of lentiviral 

inoculum at a multiplicity of infection (MOI) of 1 (1 TU per cell). As 100,000 cells per well were 
plated in manteinance medium (MEM 2% FBS), 100,000 TU must be diluted in MEM 2% FBS 

+ 5 µg/ml polybrene to a final volume of 500 μl. Incubate for 15 min at room temperature. 
4. Replace the medium of the cells with the 500 µl/well of lentiviral inoculum. Add 500 µl/well of 

MEM 2% FBS + 5 µg/ml polybrene to the control cells.  
5. Centrifuge at 300 × g for 2 h at 25 °C for viral adsorption.  

6. Replace the inoculum with 1 ml/well of MEM 2% FBS and incubate for 48 h at 37 °C and 5% 
CO2.  

7. Based on the basal background of the reporter proteins, monitor the effectiveness of the 
transduction by fluorescence microscopy in the green/GFP (FlaviA-GFP) and far-red/Cy5 

(FlaviA-mNeptune) channels. 
 

Selection 
1. For the antibiotic selection of transduced cells, replace the medium with 750 µl/well of MEM 10% 

FBS containing 8 µg/ml of puromycin (Recipe 6) and incubate overnight at 37 °C and 5% CO2. 

Apply the same treatment to the control cells.  

2. Replace the medium of both transduced and control cells with 1 ml/well of MEM 10% FBS 

containing 4 µg/ml of puromycin. Incubate at 37 °C and 5% CO2 until 100% mortality of the 

control cells is evidenced by light microscopy (commonly 24-48 h).   

3. Replace the medium of the selected cells with 1 ml/well of MEM 10% FBS + 0.5 µg/ml puromycin 

and incubate at 37 °C and 5% CO2 until reaching confluency of 80-90%.  

4. Passage the selected cells to 25 cm² culture flasks with 5 ml of MEM 10% FBS + 0.5 µg/ml 

puromycin and incubate at 37 °C and 5% CO2 until reaching a confluency of 80-90% 

(https://www.jove.com/v/5052/passaging-cells). 

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5. For the FACS selection, discard the medium, wash the cells once with 1 ml of PBS, add 500 µl 

of TrypLETM express (no phenol red), incubate for 5 min at 37 °C, and resuspend the cells with 

1 ml of PBS 1% FBS. 

6. Count the cells with a hemocytometer (https://www.jove.com/v/5048/using-a-hemacytometer-

to-count-cells) and prepare 2 ml of cell suspensions at 1,000,000 cells/ml in PBS 1% FBS. 

7. Aspirate the cell suspensions into the cell sorter. For the FlaviA-GFP reporter isolate at least 

two cell subpopulations with different but homogeneous levels of the reporter's basal 

background using the FL1 detector (488 nm laser - 530/30 nm filter) (Figure 1). Apply the same 

procedure to the FlaviA-mNeptune reporter but using the FL4 detector (640 nm laser - 675/25 

nm filter).  

Note: The basal background of the FlaviA-GFP and FlaviA-mNeptune reporters make them 

sensitive to the levels of cellular expression: If the expression is too high the background will 

mask the signal produced upon activation of the reporters. If the expression is too low there will 

not be enough reporter’s signal over the background. 

 

 
Figure 1. FACS analysis of BHK-21/FlaviA-GFP stable cells. A. Histogram showing the 

difference in the green fluorescence (FL1 detector- 530/30 nm filter) between wild-type and 

reporter BHK-21 cells due to the basal background of the FlaviA-GFP reporter proteins. B. 
Scatter plots showing the heterogeneity in the population of stable BHK-21 cells with different 

levels of expression of the FlaviA-GFP reporter. For the selection of the best reporter cells 

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(highest signal-to-noise ratio), at least two cell subpopulations with different (low, medium or 

high) but homogeneous levels of the reporter's basal background must be isolated and tested 
by live-cell imaging upon flavivirus infection. 

 

8. Seed the isolated cell suppopulations in different wells of a 48-well cell culture plate with 1 

ml/well of MEM 10% FBS + 0.5 µg/ml puromycin and incubate at 37 °C and 5% CO2 until 

reaching a confluency of 80-90%. 

9. Passage the selected cells to a 6-well cell culture plate with 3 ml of MEM 10% FBS + 0.5 µg/ml 

puromycin and incubate at 37 °C and 5% CO2 until reaching a confluency of 80-90%. 

10. Test the different isolated cell suppopulations by a live-cell imaging flavivirus infection kinetics 

according to the protocol described in Procedure C.  
Note: The best reporter cells will be those with the highest signal-to-noise ratio upon flavivirus 

infection. The fluorescence signal-to-noise ratio is calculated by dividing the signal of the 

reporter cells treated with infectious virus by the noise given by the reporter cells treated with 

UV-inactivated virus at the same post-inoculation time. 
 

C. Infection kinetics in reporter cells by live-cell imaging 
1. Prepare and titer the flaviviral seed of your choice (e.g., DENV, ZIKV, or YFV) according 

tostandard virological methodologies (Medina et al., 2012; Freppel et al., 2018). For viral 

inactivation, place 200 µl/well of the flaviviral seed in a 24-well cell culture plate, remove the lid 

and apply 5 cycles of UV light (254 nm) exposure at an energy of 400,000 µJ/cm2 into an 
ultraviolet crosslinker. Between cycles, shake the plate for 5 s using your hands.  

2. As described above, seed 15,000 BHK-21/FlaviA-GFP stable cells per well in a µClear black 
96-well plate with 100 µl/well of MEM 2% FBS and incubate overnight at 37 °C and 5% CO2. 

3. Based on the calculated titer of the flaviviral seed in plaque forming units (PFU)/ml, prepare 50 
µl/well of inoculum at a low MOI (between 0.1 and 0.25). As 15,000 cells per well were plated 

in maintenance medium, between 1,500 and 3,750 PFUs must be diluted in MEM 2% FBS to a 
final volume of 50 μl/well. Multiply for the total number of wells to be inoculated and prepare a 

single inoculum suspension. Likewise, prepare the UV-inactivated inoculum suspension.  
4. Replace the medium of the cells with 50 µl/well of either the infectious or the UV-inactivated 

flaviviral inoculum and incubate for 2 h at 37 °C and 5% CO2 for viral adsorption. Using your 
hands, shake the plate for 5 s every 15 min. 

5. Replace the inoculum with 150 µl/well of FluoroBriteTM DMEM 2% FBS (Recipe 7) and incubate 
for the desired time of your kinetics (e.g., 120 h) at 37 °C and 5% CO2 into the automated 

fluorescence microscope. Add 200 µl/well of PBS to the surrounding wells to avoid desiccation.  
6. Using your microscope’s software (e.g., Gen5 Image+), program the image acquisition with the 

4× or the 20× objective in the green/GFP channel at the desired post-infection times (Figure 2A).  
Note: The acquisition parameters (excitation intensity, exposure time, and camera gain) of the 

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images are variable according to the particular reporter cell subpopulation isolated by FACS. 

Always include an extra well of control cells for the adjustment of the acquisition parameters as 

the overexposure to the excitation light may harm the cells of the experimental conditions. Our 

recommendation is to set those parameters to a level where the background signal of the 

reporter proteins is just perceptible in the first images of the kinetics, in order to increase the 

dynamic range of the reporter’s fluorescence upon activation by flaviviral proteases.  

 

 
Figure 2. DENV-2 infection kinetics in reporter BHK-21 cells by live-cell imaging. A. Stable 

BHK-21 cells expressing the FlaviA-GFP reporter were inoculated with either infectious or UV-
inactivated DENV-2 13538 at a low MOI of 0.1 and captured by live-cell imaging at the specified 

time periods. Magnification of 40×, scale bar = 100 µm. B. The image analysis of the infection 
kinetics with the software CellProfiler 4.0 allowed the tracking of single cells over time based on 

the reported fluorescence (each colored line in the graphs corresponds to an individual cell). 
The black dashed lines represent the mean values of cell fluorescence.  

 
D. Kinetic plaque assay in reporter cells by live-cell imaging 

1. As described above, seed 25,000 BHK-21/FlaviA-mNeptune stable cells per well in a µClear 

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black 96-well plate with 100 µl/well of MEM 10% FBS and incubate overnight at 37 °C and 5% 

CO2. 
2. Prepare 10-fold serial dilutions (10-1-10-6) of the flaviviral seed in 1.5 ml reaction tubes. Start 

mixing 50 µl of the flaviviral seed in 450 µl of MEM 2% FBS (10-1). Vortex the tube for 5 s and 
mix 50 µl of the 10-1 flaviviral dilution in 450 µl of MEM 2% FBS (10-2). Repeat this procedure 

for the other dilutions (10-3-10-6). Change the tip between dilutions to avoid cross-contamination. 
For a detailed and graphical explanation of 10-fold serial dilutions preparation please refer to 
the bio-protocol paper by Freppel et al., 2018 (reference 3). 

3. Replace the medium of the cells with 50 µl/well of each serial dilution of the flaviviral seed. 

Inoculate a control well with 50 µl of UV-inactivated flaviviral seed. Incubate for 2 h at 37 °C and 
5% CO2 for viral adsorption. Using your hands, shake the plate for 5 s every 15 min.  

4. Replace the inoculum with 150 µl/well of plaque media 2% FBS (Recipe 8) and incubate for 120 
h at 37 °C and 5% CO2 into the automated fluorescence microscope. Add 200 µl/well of PBS to 

the surrounding wells to avoid desiccation.  
5. Using your microscope’s software (e.g., Gen5 Image+), program the image acquisition (a 

montage of the whole well) with the 4× objective in the far-red/Cy5 channel at the desired post-
infection times (Figure 3A).  
Note: The acquisition parameters (excitation intensity, exposure time, and camera gain) of the 

images are variable according to the particular reporter cell suppopulation isolated by FACS. 

Always include an extra well of control cells for the adjustment of the acquisition parameters, as 

the overexposure to the excitation light may harm the cells of the experimental conditions. Our 

recommendation is to set those parameters to a level where the background signal of the 

reporter proteins is just perceptible in the first images of the kinetics, in order to increase the 

dynamic range of the reporter’s fluorescence upon activation by flaviviral proteases.  

 

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Figure 3. YFV kinetic plaque assay in reporter BHK-21 cells by live-cell imaging. A. Stable 

BHK-21 cells expressing the FlaviA-mNeptune reporter were inoculated with decimal dilutions 
(10-1-10-6) of either infectious or UV-inactivated YFV 17D. After addition of plaque media 2% 

FBS, entire wells of the plate were captured by live-cell imaging at the specified time periods. 
Magnification of 40×, scale bar = 1,000 µm. B. The image analysis of the kinetic plaque assay 

with the software CellProfiler 4.0 allowed the identification of single viral plaques (upper panel) 
and the tracking of those plaques over time (lower panel). For a deeper exemplification of the 

results obtained with our kinetic plaque assay please watch the live-cell imaging video (Video 
1).  

 

 
Video 1. ZIKV plaque assay kinetics on reporter BHK-21 cells 

  

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Data analysis 
 
A. Infection kinetics in reporter cells 

Single cell tracking of infected cells based on its fluorescence (Figure 2B) was performed using our 
CellProfiler pipeline for single cell analysis (“SingleCellsTracking.cpproj”, Figure 4). To perform this 
analysis just drag and drop the images in the Images module and press Analyze Images. In order 
to modify the pipeline for your cells and conditions, go to Start Test Mode, adjust the parameters 

described in the modules (one by one) and press Step to see the output of the modifications applied 
to a particular module. Once all the modifications are ready, press Exit Test Mode and go to Analyze 

Images. The modules contained in the single cell analysis pipeline are the following:  
1. Images: Simply drag and drop the image files of a time series in the Images module. Make sure 

that the name of all the files in the dataset do include the name of the channel where the 
fluorescence was measured (e.g., GFP) and the increasing consecutive numbers for time-lapse 

microscopy images (e.g., GFP_72h).  
2. NamesAndTypes: Select the rule criteria with an expression contained in the name of all the 

files in the dataset, in this case, indicating the channel of the fluorescence (e.g., GFP). For each 

file of the dataset it creates an image called “Sensor”.  
 

 
Figure 4. CellProfiler image analysis pipeline for single cell tracking of flavivirus infected 
BHK-21/FlaviA-GFP reporter cells 

 
3. CorrectIlluminiationCalculate (Illumination function calculation: Regular): From the “Sensor” 

image, this module calculates a regular illumination correction function and creates an image 

with enhanced contrast, named “IllumSensor”. 
4. CorrectIlluminiationCalculate (Illumination function calculation: Background): From the “Sensor” 

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image, this module calculates a background-based illumination function called 

“IllumSensorbackground”. 
5. RescaleIntensity: Converts the output image of the regular illumination function (“IllumSensor”) 

to an image with rescaled intensity (“RescaleSensor”). 
6. CorrectIlluminationApply: This module applies the “IllumSensorbackground” correction function 

to the “RescaleSensor” image and generates an enhanced image named “CorrSensor”. 
7. CorrectIlluminationApply: This second module of correction works on the original “Sensor” 

image, applies the “IllumSensorbackground” correction function but keeping the original 
intensity values and generates an output image called “mSensor”. 

8. IdentifyPrimaryObjects: This module works with the enhanced image “CorrSensor” to identify 
the objects Cells. You may modify the Typical diameter to obtain the correct cell segmentation 

with other cell lines or parameters. 
9. MeasureObjectIntensity: Measures the intensities of the identified objects Cells but on the image 

with the original intensity values only corrected by illumination (“mSensor”). 
10. TrackObjects: This module tracks cells over the time-lapse microscopy and generates an output 

image called “TrackedCells”. 
11. GraytoColor, OverlayOutlines, SaveImages: These modules create and save color images with 

the outlines of the primary objects identification for documentation and validation of the cell 
segmentation by the researcher’s eye and criteria. 

12. ExportToSpreadsheet: Saves the selected measurements to an excel spreadsheet (e.g., 

Integrated intensity).  

Note: Together with this protocol we supply the Zip file “SingleCellsTracking pipeline and dataset” 

which contains the applied pipeline (“SingleCellsTracking.cpproj”) and an example dataset 

composed of a single input image to run the pipeline (“Input_image_GFP”) and two output files 

to corroborate the expected results (“Output_image_GFP” and “Infected_Cells”).  

 

B. Kinetic plaque assay in reporter cells 

The identification and tracking of viral plaques were performed using two different pipelines 

programmed in CellProfiler. For single-plaque recognition use our “PlaqueIdentification.cpproj” 
pipeline (Figure 5) to generate images such as those depicted in the upper panel of Figure 3B. To 
track the plaques over a time series and determine the cell counts for every recognized plaque, first 

apply the “PlaqueIdentification.cpproj” pipeline to generate an image with the identified plaques and 
then use that image and the “PlaqueTracking.cpproj” pipeline (Figure 6) to obtain tracking images 
such as those showed in the lower panel of Figure 3B. Depending on the cell type and/or density, 

some modifications to several parameters may be done for an optimal plaque identification using 
the option Start Test Mode and running each module step by step. The modules of the above 
mentioned pipelines are the following:  
 

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Figure 5. CellProfiler image analysis pipeline for flaviviral plaques identification in BHK-

21/mNeptune reporter cells 

 

 
Figure 6. CellProfiler image analysis pipeline for flaviviral plaques tracking in BHK-
21/mNeptune reporter cells 

 

Plaque identification pipeline 

1. Images: Simply drag and drop the image files of a time series in the Images module. Make sure 

that the name of all the files in the dataset do include the name of the channel where the 

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fluorescence was measured (e.g., mNeptune) and the increasing consecutive numbers for time-

lapse microscopy images (e.g., mNeptune_72h).  

2. NamesAndTypes: Select the rule criteria with an expression contained in the name of all the 

files in the dataset, in this case, indicating the channel of the fluorescence (e.g., mNeptune). 

For each file of the dataset it creates an image called “Sensor”. 

3. Crop: This is an optional module in case you need to remove part of the image (e.g., distance 

bars). It generates an output image named “CropSensor”. 
4. IdentifyPrimaryObjects: This module identifies the individual objects Nuclei from the 

“CropSensor” image. You may need to change the Typical diameter of objects or the Threshold 

strategy and its parameters to obtain an optimal identification of your cells. 
5. MeasureObjectNeighbors: Measures the number of neighbors for each Nuclei object within a 

specified Neighbor distance. You may need to modify this parameter to obtain a good optimal 

range of neighbor numbers to differentiate the plaque-belonging cells from the surrounding cells. 
This module creates an image called “ObjectNeighborCount”.  

6. FilterObjects: This module sets a threshold to identify plaque-belonging Nuclei objects using the 

range of number of neighbors calculated in the previous module. You may need to set this 
Minimum value according to the range of neighbors for an optimal identification of plaque 
belonging Nuclei objects. It generates the output objects FilteredNuclei.  

7. IdentifySecondaryObjects: Extends the above FilteredNuclei by a determined number of pixels 

to fill the gaps between the plaque-belonging cells in the “CropSensor” image. You may need 
to modify the Number of pixels by which to expand the primary objects in order to fill most of the 
gaps. This module identifies the output objects Cells.  

8. ConvertObjectstoImage: The expanded Cells objects constitute the basis to create a new image 

named “CellImage”. 
9. IdentifyPrimaryObjects: Uses the previous “CellImage” to identify the new Plaque objects. You 

may need to modify the range of Typical diameter of objects to obtain the correct plaque 

identification with images from different post-infection times, as shown in the colored frame 
Plaque, within the visual output generated by this module. In such an instance images must be 

analyzed one by one, like in the case of our example dataset. 
10. ConvertObjectstoImage: Converts the Plaque objects to an image called “PlaqueImage”. 

11. SaveImages: Uses the “PlaqueImage” to create and save an image called 

“Output_image_PreviousPlaques”, that constitutes one of the input images for the plaque 

tracking with the pipeline “PlaqueTracking.cpproj”.  
12. OverlayObjects: This module fuses the “CropSensor” image with the Plaque objects to make a 

composite image named “OverlayImage”. 
13. SaveImages: Creates an image called “Output_image_OverlayPlaques” based on the 

“OverlayImage”.  
Note: Together with this protocol we supply the Zip file “PlaqueIdentification tracking pipeline 

and dataset” which contains the applied pipeline (“PlaqueIdentification.cpproj”) and an example 

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dataset composed of two input images to run the pipeline and practice the required adjustments 

(“Input_image_mNeptune_72h” and “Input_image_mNeptune_96h”) and four output files to 

corroborate the expected results (“Output_image_PreviousPlaques_72h”, 

“Output_image_PreviousPlaques_96h”, “Output_image_OverlayPlaques_72h”, and 

“Output_image_OverlayPlaques_96h”).  
 

Plaque tracking pipeline 

1. Images: Simply drag and drop the files of the plaque assay fluorescence images (e.g., 

“Input_image_mNeptune_72h”) and the output images created with the previous Plaque 

identification pipeline (e.g., “Output_image_PreviousPlaques_72h”). Make sure that the name 

of the plaque assay fluorescence images do include the name of the channel where the 
fluorescence was measured (e.g., mNeptune) and the increasing consecutive numbers for time-

lapse microscopy images (e.g., mNeptune_72h). 
2. NamesAndTypes: Select the rule criteria with an expression contained in the name of all the 

plaque assay fluorescence images, in this case, indicating the channel of the fluorescence (e.g., 

mNeptune). For each fluorescence image it creates an image called “Sensor”. 
3. The modules 3-8 are the same as those described in the Plaque identification pipeline. 
4. IdentifySecondaryObjects: This module identifies the new Plaque objects in the “CellImage” as 

secondary objects around the previously identified PreviousPlaques primary objects. 
5. TrackObjects: This module tracks the plaques over time using an overlap criteria across the 

time-resolved images and creates an output image named “TrackedPlaques”. You may adjust 
the Maximum distance to consider matches for an optimal plaque tracking. 

6. SaveImages: Saves the “Tracked_Plaques” image for your validation and final results.  

7. RelateObjects: This module correlates the new Plaque objects with the previously identified 

Nuclei objects.  
8. ExporttoSpreadSheet: This module exports to an excel spreadsheet the data of the number of 

cells (Nuclei objects) that compose every recognized plaque in all the analyzed images.  

Note: Together with this protocol we supply the Zip file “PlaqueIdentification tracking pipeline 

and dataset” which contains the applied pipeline (“PlaqueTracking.cpproj”) and an example 

dataset composed of four input images to run the pipeline (“Input_image_mNeptune_72h”, 

“Input_image_mNeptune_96h”, “Output_image_Previous Plaques_72h”, and 

“Output_image_PreviousPlaques_96h”) and three output files to corroborate the expected 

results (“Tracked_Plaques_72h”, “Tracked_Plaques_96h” and “Viral_Plaque”). 

 

Recipes 
 

1. Complete DMEM  

500 ml DMEM (Gibco) 
5 ml Antibiotic-antimycotic 100× 

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5 ml (for 2%) or 50 ml (for 10%) of FBS  

Homogenize by hand rotation (20 times, gently to avoid formation of foam) 
Store at 4 °C. Stable for 4 months 

2. PEI solution (1 mg/ml) 
1 mg of PEI powder 

1 ml of HCl 0.2 M in distilled water 
Heat and shake at 60 °C, 600 rpm in a ThermoMixer® block 

Sterilize by filtration (0.2 µm pore size) 
Prepare 45 µl aliquots into 2 ml reaction tubes and store at -80° C. Stable for 4 months  

3. Polybrene solution (10 mg/ml) 
10.6 mg of hexadimethrine bromide powder  

Dissolve in 1 ml of destilled water 
Sterilize by filtration (0.2 µm pore size) 

Prepare 50 µl single use aliquots into 0.5 ml reaction tubes and store at -20 °C. Stable for 1 
year 

4. Complete MEM  
500 ml MEM (Gibco) 

5 ml Sodium pyruvate 100 mM 
5 ml Antibiotic-antimycotic 100× 

5 ml (for 2%) or 50 ml (for 10%) of FBS  
Homogenize by hand rotation (20 times, gently to avoid formation of foam) 

Store at 4 °C. Stable for 4 months  
5. PBS 1% FBS 

45 ml PBS, pH 7.4 
5 ml complete MEM 10% FBS 

Store at 4 °C. Stable for 4 months  
6. Puromycin solution (10 mg/ml) 

10 mg of puromycin  
Dissolve in 1 ml of destilled water 

Sterilize by filtration (0.2 µm pore size) 
Prepare 20 µl single use aliquots into 1.5 ml light protection reaction tubes and store at -20 °C. 

Stable for 2 years 
7. FluoroBriteTM DMEM 2% FBS 

500 ml FluoroBriteTM DMEM (Gibco) 
5 ml GlutaMAXTM supplement 

5 ml Sodium pyruvate 100 mM 
5 ml Antibiotic-antimycotic 100× 

5 ml of FBS  
Homogenize by hand rotation (20 times, gently to avoid formation of foam) 

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Store at 4 °C. Stable for 4 months  

8. Plaque media 2% FBS 
9.4 g MEM (Sigma)  

900 ml Milli-Q water 
Adjust pH to 4.0 

10 g Carboxymethylcellulose sodium salt  
Autoclave (121 °C at 100 kPa for 15 min)  

30 ml 7.5% sodium bicarbonate solution in Milli-Q water (sterilized by filtration – 0.2 µm pore 
size) 

10 ml GlutaMAXTM supplement  
10 ml Sodium pyruvate 100mM 

10 ml Antibiotic-antimycotic 100× 
20 ml of FBS 

Homogenize by hand rotation (20 times, gently to avoid formation of foam) 
Store at 4 °C. Stable for 4 months  

 
Acknowledgments 

 

We want to thank Dr. Jeanne A. Hardy from the Department of Chemistry, University of 
Massachusetts, for her kindness and scientific advice during our outstanding collaboration. We also 

want to acknowledge our funding sources at Universidad de Costa Rica (project VI-803-B9-505) 
and International Centre for Genetic Engineering and Biotechnology (Grant CRP/CRI18-02).   

 

Competing interests 
 

The authors declare that they do not have any conflicts of interests.  
 
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